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Natural C-independent expression of restriction endonuclease in a C protein-associated restriction-modification system

机译:C蛋白相关的限制性修饰系统中限制性内切酶的天然C非依赖性表达

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Restriction-modification (R-M) systems are highly prevalent among bacteria and archaea, and appear to play crucial roles in modulating horizontal gene transfer and protection against phage. There is much to learn about these diverse enzymes systems, especially their regulation. Type II R-M systems specify two independent enzymes: a restriction endonuclease (REase) and protective DNA methyltransferase (MTase). Their activities need to be finely balanced in vivo. Some R-M systems rely on specialized transcription factors called C (controller) proteins. These proteins play a vital role in the temporal regulation of R-M gene expression, and function to indirectly modulate the horizontal transfer of their genes across the species. We report novel regulation of a C-responsive R-M system that involves a C protein of a poorly-studied structural class - C.Csp231I. Here, the C and REase genes share a bicistronic transcript, and some of the transcriptional auto-control features seen in other C-regulated R-M systems are conserved. However, separate tandem promoters drive most transcription of the REase gene, a distinctive property not seen in other tested C-linked R-M systems. Further, C protein only partially controls REase expression, yet plays a role in system stability and propagation. Consequently, high REase activity was observed after deletion of the entire C gene, and cells bearing the Delta C R-M system were outcompeted in mixed culture assays by those with the WT R-M system. Overall, our data reveal unexpected regulatory variation among R-M systems.
机译:限制性修饰(R-M)系统在细菌和古细菌中非常普遍,并且似乎在调节水平基因转移和对噬菌体的保护中起关键作用。关于这些多样的酶系统,尤其是它们的调控,有很多东西要学习。 II型R-M系统指定两种独立的酶:限制性核酸内切酶(REase)和保护性DNA甲基转移酶(MTase)。他们的活动需要在体内达到良好的平衡。一些R-M系统依赖于称为C(控制蛋白)蛋白的专门转录因子。这些蛋白质在R-M基因表达的时间调控中起着至关重要的作用,并起到间接调节其基因在整个物种中水平转移的作用。我们报告的C响应R-M系统涉及一个研究程度不高的结构类别-C.Csp231I的C蛋白的新型调节。在这里,C和REase基因共享双顺反子转录物,并且在其他C调控的R-M系统中看到的某些转录自动控制功能得以保留。但是,单独的串联启动子驱动REase基因的大多数转录,这是在其他经过测试的C连接的R-M系统中未发现的独特特性。此外,C蛋白仅部分控制REase的表达,但在系统稳定性和繁殖中起作用。因此,在缺失整个C基因后观察到了高的REase活性,并且具有WT C-M系统的细胞在混合培养试验中比具有Delta C R-M系统的细胞更胜一筹。总体而言,我们的数据揭示了R-M系统之间意想不到的监管差异。

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